Article Figures & Data

Figures

The genome is organized through a hierarchy of long-range interactions. A, large chromosomal neighborhoods associate with each other in the nuclear space. Euchromatic regions that are associated with high transcriptional activity tend to cluster in the center of the nucleus. In contrast, heterochromatic regions associated with transcriptional repression tend to cluster at the nuclear periphery. B, heat map representing virtual genome-wide chromatin interaction maps. Megabase scale chromatin interaction partitions the genome into domains of interactions known as topologically associated domains (TAD). TAD boundaries preclude interactions between neighboring TADs, therefore restricting most interactions to within their borders. C, enhancer–promoter chromatin interactions are mediated by the chromatin interaction factors ZNF143 and CTCF, in concert with several accessory/cobinding proteins. These factors act in concert with several cobinding/accessory/associated proteins to influence genome organization via enhancer–promoter interactions. Enhancer–promoter interactions are at the kilobase (Kb) scale and are highly cell-type specific. D, anchors of chromatin interactions that define TAD boundaries are enriched for CTCF and cohesin binding. TADs are up to a megabase (Mb) in scale and are highly conserved across cell types.

Genetic and epigenetic alterations are observed at gene promoters in cancer. A, alterations in the sequences of promoters can modulate transcription factor binding affinity for the DNA to change the expression of the associated gene. This can arise through somatic mutations or inherited SNVs. B, changes in the epigenetic identity, based on either changes in the DNA methylation or histone modifications, were reported in cancer initiation and progression that influence promoter activity and result in altered gene expression in cancer. Open circles, unmethylated; closed circles, methylated.

Genetic and epigenetic alterations are observed at enhancers in cancer. A, SNVs and structural variations can alter enhancer activity. SNVs and somatic mutations observed in enhancers can modulate the activity of these regulatory elements by changing their affinity for transcription factors. Translocation of a region that acts as an enhancer that places it in proximity of an oncogene can drive its aberrant expression. Similarly, amplification of an active enhancer element that is associated with an oncogene can drive its overexpression and subsequently contribute to oncogenesis. These genetic alterations to enhancers ultimately serve to modulate expression of oncogenes or tumor-suppressor genes. B, changes in the epigenetic identity have been reported at enhancers in cancer. Hypermethylation or hypomethylation of CpGs at enhancers affects the accessibility of the DNA to transcription factors. Changes in the composition of post-translational modifications to histones in enhancers are thought to affect transcription factor binding to the chromatin. Increased histone acetylation increases chromatin accessibility to favor transcription factor binding, whereas loss of acetylation decreases chromatin accessibility, thereby modulating the activity of enhancers. Open circles, unmethylated; closed circles, methylated.

Genetic and epigenetic alterations targeting anchors of chromatin interactions. A, ZNF143 recognizes a DNA binding motif that is enriched at promoters. Genetic alteration in the consensus motif of ZNF143 can deter ZNF143 binding, resulting in the impaired chromatin interactions between promoters and enhancers and affecting the expression of target genes. B, anchors of chromatin interactions that define TADs are bound by CTCF. Disruption of CTCF binding at these anchors can abrogate the formation of chromatin interactions to ultimately disrupt the three-dimensional organization of the genome in cancer. CTCF recognizes a 12–base pair (bp) consensus motif mutated in various cancer types. The binding of CTCF to the DNA can also be compromised by DNA methylation, as reported in glioblastoma.